Fatty acid free bsa

Manufactured by MP Biomedicals

Sourced in Macao

Fatty acid free bovine serum albumin (BSA) is a highly purified protein derived from bovine serum. It is processed to remove any fatty acids that may be present. The core function of fatty acid free BSA is to provide a protein source that is free of interfering lipids for use in various laboratory applications.

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Lab products found in correlation

Hyclone dmem medium, by Thermo Fisher Scientific (1 mentions) Negative magnetic selection, by Miltenyi Biotec (1 mentions) Interleukin 7 (il 7), by BioLegend (1 mentions) Fatty acids, by Nu-Chek Prep (1 mentions) Nbd ps, by MP Biomedicals (1 mentions) Sodium dithionite, by Merck Group (1 mentions) Fortessa, by BD (1 mentions) Nbd ps, by Avanti Polar Lipids (1 mentions) Nbd pc, by Avanti Polar Lipids (1 mentions)

4 protocols using fatty acid free bsa

Estrogen and Palmitate Treatment Protocol

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N43 cells (CELLutions Biosystem Inc., Cedarlane, Burlington, NC, USA) and BV2 cells (gift from C.K. Glass) were cultured in HyClone^™ DMEM medium (Thermo Scientific), containing 10% charcoal:dextran stripped fetal bovine serum (Gemini, West Sacramento, CA) 100 units/mL penicillin G sodium and 100 μg/mL streptomycin sulfate and 100 mg/L sodium pyruvate. Cells were grown for 24 h before treatments with medium containing 2% charcoal:dextran stripped fetal bovine serum. Cells were pretreated for the indicated time with 10⁻⁸ M E2 (Sigma, St-Louis, MO) conjugated with fatty acid free BSA (MP Biomedicals, LLC, Solon, OH) and then treated for 8 h with 10⁻⁸ M E2 or 100 μM PA (Matreya, Pleasant Gap, PA) conjugated with BSA alone or in combination.

Morselli E., Fuente-Martin E., Finan B., Kim M., Frank A., Garcia-Caceres C., Navas C.R., Gordillo R., Neinast M., Kalainayakan S.P., Gao Y., Yi C.X., Hahner L., Palmer B.F., Tschöp M.H, & Clegg D.J. (2014). Hypothalamic PGC-1α Protects Against High Fat Diet Exposure by Regulating ERα. Cell reports, 9(2), 633-645.

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Modulating CD8+ T Cell Activation

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Naïve CD8⁺ T cells were isolated from the spleens
of 13-15 week old female wildtype or OT-1 mice using negative magnetic
selection (Miltenyi Biotec) and stained with Cell Trace Violet (CTV,
ThermoFisher Scientific) as per the manufacturer’s instructions.
50,000 CD8⁺ T cells were plated per well on 96-well plates
pre-coated with αCD3/αCD28 antibodies at concentrations
ranging from 0 to 8 μg/mL and incubated at 37°C in a
humidified 5% CO₂ incubator. For free fatty acid supplementation,
palmitate and oleate were individually conjugated to fatty acid-free BSA (MP
Biomedicals) in 150 mM NaCl at a 6:1 molar ratio to make a 4 mM, pH-adjusted
FA stock solution. For fatty acid supplementation, 100 μM each of
BSA-conjugated palmitate and oleate was added to the culture medium
containing charcoal-stripped serum, or an equivalent concentration of BSA
alone as a control. After 48-72 hours of stimulation, cell numbers,
viability, and proliferation were measured by flow cytometry. A naïve
control was maintained with 10 ng/mL IL-7 (BioLegend).

Ringel A.E., Drijvers J.M., Baker G.J., Catozzi A., García-Cañaveras J.C., Gassaway B.M., Miller B.C., Juneja V.R., Nguyen T.H., Joshi S., Yao C.H., Yoon H., Sage P.T., LaFleur M.W., Trombley J.D., Jacobson C.A., Maliga Z., Gygi S.P., Sorger P.K., Rabinowitz J.D., Sharpe A.H, & Haigis M.C. (2020). Obesity shapes metabolism in the tumor microenvironment to suppress anti-tumor immunity. Cell, 183(7), 1848-1866.e26.

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Preparation of Fatty Acid-BSA Conjugates

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Fatty acids were purchased from NuChek Prep (Waterville, MN). Fatty acid free BSA was purchased from MP Bio-medicals. Fatty acids were made into fatty acid-BSA conjugate solution (5 mM). Briefly, Fatty acids were saponified with NaOH at 70 °C for 30 min and then mixed with 6 % Fatty acid free BSA dissolved in PBS. 5 mM stock solutions were stored in aliquots at −20 °C [20 (link)]. These fatty acid-BSA conjugates were also routinely analyzed by GC with flame ionization detection of their acid methanolysis products [21 (link)] to confirm the concentration and identity of the purity of the fatty acid molecular species. These fatty acid-BSA conjugates were dissolved in cell culture media to desired concentrations immediately prior to use in experiments.

Shao F, & Ford D.A. (2014). Elaidic Acid Increases Hepatic Lipogenesis by Mediating Sterol Regulatory Element Binding Protein-1c Activity in HuH-7 Cells. Lipids, 49(5), 403-413.

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Quantifying Lipid Flippase and Scramblase Activity

Cited 1 time

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Flippase was measured as previously described [14 (link)]. Briefly, cells were resuspended in 3ml of flippase assay buffer and NBD-PS (Avanti Polar Lipids) was added to a final concentration of 3 μM. Cells with NBD-PS were divided into aliquots and incubated for 0, 1, 5, 15, 30 or 45 minutes. After each incubation time, half of the cell suspension was separated for non-extracted sample and kept on ice. The remaining half was spun down to remove non inserted NBD-PS and subjected to BSA extraction of NBD-PS from the outer leaflet by adding 3% fatty acid free BSA (MP Biomedicals) in flippase assay buffer. After incubation on ice for 20 minutes, freshly prepared sodium dithionite (Sigma) was added to a final concentration of 10 mM and incubated a further 10 minutes, to reduce the NBD lipids in the outer cell surface. The cells were spun down and resuspended in flippase assay buffer containing 0.25% BSA and 2 μg/ml PI. NBD-PS signal from unextracted and extracted samples was measured by flow cytometry from living cells after exclusion of PI-positive dead cells, using a BD Fortessa. Non-extractable NBD-PS in the BSA and sodium dithionite treated sample was presented as the percentage of total amount in the control unextracted sample. Scramblase was measured in the same way but with NBD-PC (Avanti Polar Lipids).

Davis H.W., Vallabhapurapu S.D., Chu Z., Vallabhapurapu S.L., Franco R.S., Mierzwa M., Kassing W., Barrett W.L, & Qi X. (2019). Enhanced phosphatidylserine-selective cancer therapy with irradiation and SapC-DOPS nanovesicles. Oncotarget, 10(8), 856-868.

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